CN107384832B - Method for culturing nitrogen-fixing blue algae in large quantity at low cost - Google Patents

Method for culturing nitrogen-fixing blue algae in large quantity at low cost Download PDF

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CN107384832B
CN107384832B CN201710755178.0A CN201710755178A CN107384832B CN 107384832 B CN107384832 B CN 107384832B CN 201710755178 A CN201710755178 A CN 201710755178A CN 107384832 B CN107384832 B CN 107384832B
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彭成荣
张金丽
张云
黄顺
宋学宁
李敦海
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Abstract

The invention discloses a method for culturing nitrogen-fixing blue algae in large quantity at low cost, which comprises the following steps: 1. collecting livestock and poultry breeding waste and carrying out solid-liquid separation to obtain a livestock and poultry breeding waste separation solution; 2. determining the content of total nitrogen and total phosphorus in the livestock and poultry breeding waste separation liquid; 3. diluting the livestock and poultry breeding waste separation liquid; 4. domesticating and culturing nitrogen-fixing blue algae and collecting algae seeds; 5. preparing a simple nitrogen fixing cyanobacteria culture medium JYM; 6. mixing the livestock and poultry breeding waste separation diluent with a JYM culture medium in a volume ratio of 1:1.5-9:1 to prepare a low-cost nitrogen fixing blue algae culture medium; 7. the domesticated nitrogen-fixing blue algae is treated with OD680And =0.1-0.3, inoculating the strain into a low-cost azotobacter culture medium for natural culture. The method is simple and easy to implement, has low cost, reasonably utilizes livestock and poultry breeding waste, and realizes the low-cost culture of the nitrogen-fixing blue algae.

Description

Method for culturing nitrogen-fixing blue algae in large quantity at low cost
Technical Field
The invention belongs to the technical field of bioengineering, relates to culture of microalgae biomass, and more particularly relates to a method for culturing nitrogen-fixing blue algae in large quantities at low cost.
Background
Nitrogen fixing blue algae belongs to the Cyanophyta (Cyanophyta) and is the most primitive of algae plants. It can fix molecular nitrogen in the air into nitrogen compounds which can be utilized by crops through differentiated heteromorphic cells. Since Frank of Germany in 1889 discovered that certain algae have biological characteristics of nitrogen fixation, people begin to consciously recognize and utilize nitrogen-fixing blue algae for agricultural production. Until 90 s in the 20 th century, more than 150 kinds of algae of 33 genera have been reported to have nitrogen fixing capability all over the world, and most of the reported nitrogen-fixing blue algae belong to the genera Nostoc and Anabaena.
China produces 21% of grains in the world by 8% of cultivated land in the world, but the consumption of chemical fertilizers accounts for 35% of the world. The amount of the homogenized fertilizer per mu in China is 21.9 kilograms, which is far higher than the average level in the world (8 kilograms per mu), and is 2.6 times of that in the United states and 2.5 times of that in European Union. With the gradual increase of the fertilizer dosage, a series of problems of soil hardening, soil acidification and the like cause the gradual degradation of cultivated land in China. The nitrogen-fixing property and the self living property of the nitrogen-fixing blue algae enable the nitrogen-fixing blue algae to have wide application space in the aspect of cultivation of agricultural crops. The nitrogen-fixing blue algae is used as a crop fertilizer source, so that nitrogen can be provided for crops, the use of nitrogen fertilizer is reduced, organic matters in soil can be increased, the soil is improved, and active substances can be provided to promote the growth of the crops. Therefore, the utilization of the nitrogen-fixing blue algae as a fertilizer source is beneficial to solving a series of ecological environment problems of soil hardening, soil acidification and water body pollution caused by excessive application of chemical fertilizer.
Although nitrogen-fixing cyanobacteria has a wide prospect in agricultural production, large-scale culture of nitrogen-fixing cyanobacteria faces a cost challenge because the culture process of nitrogen-fixing cyanobacteria needs to consume more chemical reagents. China is a big livestock and poultry breeding country, the total meat yield is the first world, meat 1/3 is produced in China globally, and a large amount of waste generated by livestock and poultry breeding cannot be deeply utilized and then is discharged out of order, so that the problem of serious environmental pollution is caused. Therefore, the rational utilization of livestock and poultry breeding waste for large-scale culture of nitrogen-fixing blue algae can play a positive role in agricultural non-point source pollution treatment.
Disclosure of Invention
In order to solve the problems in the prior art, the invention aims to provide a method for culturing nitrogen-fixing blue algae in large quantity at low cost, which has the advantages of easy method, low cost and simple and convenient operation, reasonably utilizes livestock and poultry breeding waste, and realizes the low-cost culture of the nitrogen-fixing blue algae.
In order to achieve the purpose, the invention adopts the following technical scheme:
a method for culturing nitrogen-fixing blue algae in large quantity at low cost comprises the following steps:
1. livestock and poultry breeding waste collection and pretreatment: collecting livestock and poultry breeding waste from a farm, mixing solid excrement and liquid excrement and performing solid-liquid separation to obtain livestock and poultry breeding waste separation liquid;
2. determining the nutrient parameters of the livestock and poultry breeding waste separation liquid: measuring the total nitrogen content and the total phosphorus content in the livestock and poultry breeding waste separation liquid to obtain the total nitrogen content C1mg/L and the total phosphorus content C2 mg/L;
3. diluting the livestock and poultry breeding waste separation liquid: respectively calculating the dilution ratio of the livestock and poultry breeding waste separation liquid by using the total nitrogen content C1 and the total phosphorus content C2, wherein the calculation formula is as follows:
livestock and poultry breeding waste separation liquid dilution ratio based on total nitrogen:
Figure BDA0001391068670000021
livestock and poultry breeding waste separation liquid dilution ratio based on total phosphorus:
Figure BDA0001391068670000022
comparing the sizes of D1 and D2, if D1 is greater than D2, diluting the livestock and poultry breeding waste separating medium according to the numerical value of D2, otherwise, diluting the livestock and poultry breeding waste separating medium according to the numerical value of D1 to obtain a livestock and poultry breeding waste separating diluent;
4. domestication culture of nitrogen-fixing blue algae and collection of algae seeds: ventilating and culturing nitrogen-fixing blue algae to logarithmic growth phase by using a liquid BG11 culture medium, naturally settling to remove supernatant to obtain algae slurry, diluting the livestock and poultry breeding waste separation diluent by 100 times again, adding the diluted diluent into the algae slurry to make the volume of the algae slurry consistent with that before removing the supernatant, and naturally settling to remove the supernatant after ventilating and culturing for 36-48 hours to obtain domesticated algae slurry;
5. preparing a simple nitrogen fixing cyanobacteria culture medium JYM: based on calcium magnesium phosphate fertilizer, trace elements are added to prepare a simple low-cost nitrogen fixing cyanobacteria culture medium, and the formula is as follows: commercial calcium magnesium phosphate fertilizer 1.12 g.L-1、1.43mg·L-1Boric acid (H)3BO3)、0.93mg·L-1Manganese chloride tetrahydrate (MnCl)2·4H2O)、0.195mg·L-1Sodium molybdate dihydrate (Na)2MoO4·2H2O)、0.11mg·L-1Zinc sulfate heptahydrate (ZnSO)4·7H2O)、0.04mg·L-1Cupric sulfate pentahydrate (CuSO)4·5H2O)、0.025mg·L-1Cobalt nitrate hexahydrate (Co (NO)3)2·6H2O);
6. Preparing a low-cost nitrogen-fixing cyanobacteria culture medium: mixing the livestock and poultry breeding waste separation diluent in the step 3 with a simple nitrogen-fixing blue algae culture medium JYM according to the volume ratio of 1:1.5-9:1 to prepare a low-cost nitrogen-fixing blue algae culture medium;
7. inoculating and culturing the domesticated nitrogen-fixing blue algae: OD of domesticated nitrogen-fixing blue algae slurry680Inoculating the strain into a low-cost azotobacter culture medium for natural culture, namely performing open culture by adopting natural illumination, and stirring every 16 to 24 hours in the culture process;
the nitrogen-fixing blue algae is any one of Nostoc, Tolypochorix or Anabaena.
Preferably, when any one of anabaena is selected for culture, the low-cost blue algae culture medium in the step 6) is mixed according to the volume ratio of the livestock and poultry breeding waste separation diluent to the simple blue algae culture medium JYM of 1: 1.5.
Preferably, when any one of the monarda is selected for culturing, the low-cost nitrogen-fixing blue algae culture medium in the step 6) is mixed according to the volume ratio of the livestock and poultry breeding waste separation diluent to the simple nitrogen-fixing blue algae culture medium JYM of 1:1.
Preferably, when any one of nostoc is selected for culture, the low-cost nitrogen-fixing blue algae culture medium in the step 6) is mixed according to the volume ratio of 9:1 of the livestock and poultry breeding waste separation diluent to the simple nitrogen-fixing blue algae culture medium JYM.
Compared with the prior art, the invention has the following advantages and effects:
1. the method for culturing the nitrogen-fixing blue algae in large scale can realize deep and efficient utilization of livestock and poultry breeding wastes.
2. The nitrogen-fixing blue algae is cultured by the low-cost nitrogen-fixing blue algae culture medium, so that the culture cost of the nitrogen-fixing blue algae is greatly reduced, and the nitrogen-fixing blue algae can be widely applied to agricultural production.
Drawings
FIG. 1 is a growth curve of FACHB-119 in various media.
FIG. 2 growth curves of FACHB-176 in different media.
FIG. 3 growth curves of FACHB-179 in different media.
FIG. 4 growth curves of FACHB-129 in different media.
FIG. 5 growth curves of FACHB-148 in different media.
Detailed Description
Example 1:
the method for culturing the nitrogen-fixing blue algae in large quantity at low cost by taking anabaena as an example comprises the following steps:
1. livestock and poultry breeding waste collection and pretreatment: collecting breeding waste from a certain pig farm in the city of Tanzhou, Hubei, mixing solid excrement and liquid manure, and performing solid-liquid separation by using a plate and frame filter press to obtain pig manure separation liquid, wherein the residual solid waste can be subjected to fertilizer-based resource utilization.
2. And (3) determining the nutrient parameters of the pig manure separation liquid: and (3) determining the total nitrogen and total phosphorus contents of the pig manure separation liquid by referring to the methods of national environmental protection standards HJ 636-2012 and HJ 671-2013, and obtaining the total nitrogen content C1-2107.40 mg/L and the total phosphorus content C2-195.24 mg/L.
3. Diluting a pig manure separation liquid: respectively calculating the dilution ratio of the livestock and poultry breeding waste separation liquid by using the total nitrogen content C1 and the total phosphorus content C2, wherein the calculation formula is as follows:
dilution factor of pig manure separation liquid based on total nitrogen:
Figure BDA0001391068670000041
dilution factor of pig manure separation liquid based on total phosphorus:
Figure BDA0001391068670000042
and comparing the sizes of D1 and D2, if D1 is greater than D2, diluting the livestock and poultry breeding waste separating medium according to the numerical value of D2, and otherwise, diluting the livestock and poultry breeding waste separating medium according to the numerical value of D1 to obtain the livestock and poultry breeding waste separating and diluting solution. Because D2 is more than D1, the pig manure separation liquid is diluted by 8.5 times to obtain the pig manure separation dilution liquid.
4. Domestication culture of nitrogen-fixing blue algae and collection of algae seeds: performing aeration culture on Anabaena azotica FACHB-119(Anabaena azotica), Anabaena FACHB-176(Anabaena sp.1058) and Anabaena FACHB-179(Anabaena sp.1105) in a liquid BG11 culture medium in a 10L serum bottle until the logarithmic phase is reached, and naturally settling to remove most of supernatant to obtain algae slurry; and (3) diluting the pig manure separation diluent by 100 times again, adding the diluted pig manure separation diluent into the algae slurry to enable the volume of the algae slurry to be consistent with that before the supernatant is removed, ventilating and culturing for 36-48 hours, naturally settling for 12 hours, and removing most of the supernatant to obtain domesticated FACHB-119, FACHB-176 and FACHB-179 algae slurry.
The Algae are all taken from fresh water Algae seed bank (Freewater Algae Current Collection of the Institute of Hydrobiology, FACHB-collection) of Chinese academy of sciences.
The culture conditions are specifically as follows: the temperature is 28-30 deg.C day, the temperature is 20-25 deg.C night, the light-dark period is 12/12 hr, and the illumination intensity is 70-100 μmol · m-2·s-1
The aeration culture is carried out by pumping gas into liquid culture medium with air pump, filtering air with Millipore Millex-GP filter before introducing gas into culture medium, wherein the aeration rate is 9. L.h-1
The formula of the BG11 culture medium is as follows: 1500 mg. L-1Sodium nitrate (NaNO)3)、75mg·L-1Magnesium sulfate heptahydrate (MgSO)4·7H2O)、40mg·L-1Dipotassium hydrogen phosphate trihydrate (K)2HPO3·3H2O)、36mg·L-1Calcium chloride dihydrate (CaCl)2·2H2O)、20mg·L-1Sodium carbonate (Na)2CO3)、6mg·L-1Citric acid (C)6H8O7)、6mg·L-1Ferric ammonium citrate (C)6H10FeNO8)、1mg·L-1Disodium ethylene diamine tetraacetate (EDTA-Na)2)、2.86mg·L-1Boric acid (H)3BO3)、1.86mg·L-1Manganese chloride tetrahydrate (MnCl)2·4H2O)、0.39mg·L-1Sodium molybdate dihydrate (Na)2MoO4·2H2O)、0.22mg·L-1Zinc sulfate heptahydrate (ZnSO)4·7H2O)、0.08mg·L-1Cupric sulfate pentahydrate (CuSO)4·5H2O)、0.05mg·L-1Cobalt nitrate hexahydrate (Co (NO)3)2·6H2O)。
5. Preparing a simple nitrogen fixing cyanobacteria culture medium JYM: based on calcium magnesium phosphate fertilizer, trace elements are added to prepare a simple low-cost nitrogen fixing cyanobacteria culture medium, and the formula is as follows: commercial calcium magnesium phosphate fertilizer 1.12 g.L-1、1.43mg·L-1Boric acid (H)3BO3)、0.93mg·L-1Manganese chloride tetrahydrate (MnCl)2·4H2O)、0.195mg·L-1Sodium molybdate dihydrate (Na)2MoO4·2H2O)、0.11mg·L-1Zinc sulfate heptahydrate (ZnSO)4·7H2O)、0.04mg·L-1Cupric sulfate pentahydrate (CuSO)4·5H2O)、0.025mg·L-1Cobalt nitrate hexahydrate (Co (NO)3)2·6H2O)。
6. Different nitrogen fixing blue algae culture media are prepared according to the following method:
(1) mixing the pig manure separation diluent with a simple nitrogen-fixing blue algae culture medium JYM according to the volume ratio of 1:1.5 to prepare a low-cost nitrogen-fixing blue algae culture medium;
(2) directly separating the diluent by using pig manure;
(3) BG11 medium was used directly.
7. Inoculating and culturing domesticated FACHB-119, FACHB-176 and FACHB-179 algae slurry: domesticated FACHB-119, FACHB-176 and FACHB-179 algal slurry according to OD680Inoculating 0.3 of the culture medium into different culture media in step 6 for natural cultureAnd (3) carrying out open culture by using natural illumination, and stirring once every 16-24 hours in the culture process, so that the growth of the nitrogen-fixing blue algae is not influenced by natural sedimentation. The chlorophyll a concentration is measured every 2 days in the culture process to draw the growth curve of the chlorophyll a under different culture conditions.
As can be seen from FIG. 1, the algal biomass obtained by using the low-cost Anabaena azotobacter culture medium is not significantly different from that obtained by using BG11 culture medium for Anabaena azotica FACHB-119. The biomass of the algae obtained by separating the diluent by the pig manure is far lower than that of the two culture mediums. The difference in algal biomass obtained for the three media was not significant for anabaena FACHB-176 (fig. 2). For anabaena FACHB-179, the algae biomass obtained by using the low-cost nitrogen-fixing cyanobacteria culture medium is much higher than that of BG11 culture medium and pig manure separation diluent (fig. 3). In conclusion, for anabaena azotica, the low-cost anabaena azotica culture medium prepared by mixing the livestock and poultry breeding waste separation diluent and the simple type anabaena azotica culture medium JYM according to the ratio of 1:1.5 can obtain the algae biomass equivalent to or higher than that of the traditional BG11 culture medium under the same culture condition, and meanwhile, the cost of microalgae culture can be obviously reduced.
Example 2:
the method for culturing nitrogen-fixing blue algae in large quantity at low cost by taking the small unicellular algae as an example comprises the following steps:
1. livestock and poultry farming waste collection and measurement were the same as in example 1.
2. And according to the measurement result, diluting the pig manure separation liquid by 50 times for later use.
3. Domestication culture of nitrogen-fixing blue algae and collection of algae seeds: bifidobacterium breve FACHB-129 (Tolypotrix tenuis) was cultured in a 10L serum bottle with aeration using liquid BG11 medium until logarithmic phase, and algal slurry was obtained after removing most of the supernatant by natural sedimentation. And (3) diluting the pig manure separation diluent by 100 times again, adding the diluted pig manure separation diluent into the algae slurry to enable the volume of the algae solution to be consistent with that before the supernatant is removed, ventilating and culturing for 36-48 hours, naturally settling for 12 hours, and removing most of the supernatant to obtain the domesticated FACHB-129 algae slurry.
The algal species is taken from fresh water algal species Bank (Freshwater Algae Culture Collection of Hydrobiology, FACHB-collection) of Chinese academy of sciences.
The culture conditions are specifically as follows: the temperature is 28-30 deg.C day, 20-25 deg.C night, the light-dark period is 12/12 hr, and the illumination intensity is 70-100 μmol m-2s-1
The aeration culture conditions were the same as in example 1.
The BG11 medium formulation was the same as in example 1.
4. The configuration of the simple cyanobacteria fixing medium JYM is the same as that in example 1.
5. Different nitrogen fixing blue algae culture media are prepared according to the following method:
(1) preparing a low-cost nitrogen-fixing cyanobacteria culture medium: mixing the pig manure separation diluent with a simple nitrogen fixing blue algae culture medium JYM according to the volume ratio of 1:1 to prepare a low-cost nitrogen fixing blue algae culture medium;
(2) directly separating the diluent by using pig manure;
(3) BG11 medium was used directly.
6. Inoculating and culturing domesticated FACHB-129 algae slurry: the domesticated FACHB-129 algae slurry is according to OD680Respectively inoculating 0.1 of the total nutrient into different culture media in the step 5 for natural culture, namely adopting natural illumination to carry out open culture, and stirring once every 16-24 hours in the culture process so as to prevent the nitrogen-fixing blue algae from influencing the growth due to natural sedimentation. The chlorophyll a concentration is measured every 2 days in the culture process to draw the growth curve of the chlorophyll a under different culture conditions.
As can be seen from fig. 4, for the bifidobacterium parvum FACHB-129, the low-cost nitrogen-fixing blue algae culture medium prepared by mixing the livestock and poultry breeding waste separation diluent and the simple nitrogen-fixing blue algae culture medium JYM according to the ratio of 1:1 can obtain about 10% lower algae biomass than the traditional BG11 culture medium under the same culture conditions, but can obviously reduce the cost of microalgae culture.
Example 3:
the method for culturing nitrogen-fixing blue algae in large quantity at low cost by taking nostoc as an example comprises the following steps:
1. livestock and poultry farming waste collection and measurement were the same as in example 1.
2. And according to the measurement result, diluting the pig manure separation liquid by 50 times for later use.
3. Domestication culture of nitrogen-fixing blue algae and collection of algae seeds: nostoc sp (Nostoc sp.) Nostoc is cultured in 10L serum flasks with aeration to logarithmic growth phase in liquid BG11 medium, and algal slurry is obtained after removing most of the supernatant by natural sedimentation. And (3) diluting the pig manure separation diluent by 100 times again, adding the diluted pig manure separation diluent into the algae slurry to enable the volume of the algae solution to be consistent with that before the supernatant is removed, ventilating and culturing for 36-48 hours, naturally settling for 12 hours, and removing most of the supernatant to obtain the domesticated FACHB-148 algae slurry.
The algal species is taken from fresh water algal species Bank (Freshwater Algae Culture Collection of Hydrobiology, FACHB-collection) of Chinese academy of sciences.
The culture conditions are specifically as follows: the temperature is 28-30 deg.C day, 20-25 deg.C night, the light-dark period is 12/12 hr, and the illumination intensity is 70-100 μmol m-2s-1
The aeration culture conditions were the same as in example 1.
The BG11 medium formulation was the same as in example 1.
4. The configuration of the simple cyanobacteria fixing medium JYM is the same as that in example 1.
5. Different nitrogen fixing blue algae culture media are prepared according to the following method:
(1) preparing a low-cost nitrogen-fixing cyanobacteria culture medium: mixing the pig manure separation diluent with a simple nitrogen fixing blue algae culture medium JYM according to the volume ratio of 9:1 to prepare a low-cost nitrogen fixing blue algae culture medium;
(2) directly separating the diluent by using pig manure;
(3) BG11 medium was used directly.
6. Inoculating and culturing domesticated FACHB-148 algae slurry: the domesticated FACHB-148 algal slurry is according to OD680Inoculating 0.1 of the strain into different culture media in the step 5 for natural culture, namely performing open culture by using natural illuminationAnd stirring every 16-24 hours in the culture process, so that the growth of the nitrogen-fixing blue algae cannot be influenced by natural sedimentation. The chlorophyll a concentration is measured every 2 days in the culture process to draw the growth curve of the chlorophyll a under different culture conditions.
As can be seen from fig. 5, for nostoc FACHB-148, the low-cost dunaliella salina culture medium prepared by mixing the livestock and poultry breeding waste separation diluent and the simple dunaliella salina culture medium JYM according to the ratio of 9:1 can obtain 17% lower algae biomass than the traditional BG11 culture medium under the same culture conditions, but can significantly reduce the cost of microalgae culture.
The specific examples described herein are merely illustrative of the spirit of the present invention, and the method of culturing nitrogen-fixing cyanobacteria in large quantities at low cost according to the present invention can also be applied to any of the genera Nostoc, Tolypochorix, or Anabaena. Various modifications or additions may be made to the described embodiments or alternatives may be employed by those skilled in the art without departing from the spirit or ambit of the invention as defined in the appended claims.

Claims (4)

1. A method for culturing nitrogen-fixing blue algae in large quantity at low cost comprises the following steps:
1) livestock and poultry breeding waste collection and pretreatment: collecting livestock and poultry breeding waste from a farm, mixing solid excrement and liquid excrement and performing solid-liquid separation to obtain livestock and poultry breeding waste separation liquid;
2) determining the nutrient parameters of the livestock and poultry breeding waste separation liquid: measuring the total nitrogen content and the total phosphorus content in the livestock and poultry breeding waste separation liquid to obtain the total nitrogen content C1mg/L and the total phosphorus content C2 mg/L;
3) diluting the livestock and poultry breeding waste separation liquid: respectively calculating the dilution ratio of the livestock and poultry breeding waste separation liquid by using the total nitrogen content C1 and the total phosphorus content C2, wherein the calculation formula is as follows:
livestock and poultry breeding waste separation liquid dilution ratio based on total nitrogen:
Figure FDA0001391068660000011
livestock and poultry breeding waste separation liquid dilution ratio based on total phosphorus:
Figure FDA0001391068660000012
comparing the sizes of D1 and D2, if D1 is greater than D2, diluting the livestock and poultry breeding waste separating medium according to the numerical value of D2, otherwise, diluting the livestock and poultry breeding waste separating medium according to the numerical value of D1 to obtain a livestock and poultry breeding waste separating diluent;
4) domestication culture of nitrogen-fixing blue algae and collection of algae seeds: ventilating and culturing nitrogen-fixing blue algae to logarithmic growth phase by using a liquid BG11 culture medium, naturally settling to remove supernatant to obtain algae slurry, diluting the livestock and poultry breeding waste separation diluent by 100 times again, adding the diluted diluent into the algae slurry to make the volume of the algae slurry consistent with that before removing the supernatant, and naturally settling to remove the supernatant after ventilating and culturing for 36-48 hours to obtain domesticated algae slurry;
5) preparing a simple nitrogen fixing cyanobacteria culture medium JYM: based on calcium magnesium phosphate fertilizer, trace elements are added to prepare a simple low-cost nitrogen fixing cyanobacteria culture medium, and the formula is as follows: commercial calcium magnesium phosphate fertilizer 1.12 g.L-1、1.43mg·L-1Boric acid, 0.93 mg. L-1Manganese chloride tetrahydrate, 0.195 mg.L-1Disodium molybdate dihydrate, 0.11 mg.L-10.04 mg.L of zinc sulfate heptahydrate-1Blue vitriod, 0.025 mg.L-1Cobalt nitrate hexahydrate;
6) preparing a low-cost nitrogen-fixing cyanobacteria culture medium: mixing the livestock and poultry breeding waste separation diluent in the step 3) with a simple nitrogen cyanobacteria culture medium JYM according to a volume ratio of 1:1.5-9:1 to prepare a low-cost nitrogen cyanobacteria culture medium;
7) inoculating and culturing the domesticated nitrogen-fixing blue algae: OD of domesticated nitrogen-fixing blue algae slurry680Inoculating the strain into a low-cost azotobacter culture medium for natural culture, namely performing open culture by adopting natural illumination, and stirring every 16 to 24 hours in the culture process;
the nitrogen-fixing blue algae is any one of Nostoc, Dioscorea or Anabaena of Cyanophyta.
2. The method for culturing nitrogen-fixing cyanobacteria in large quantity at low cost according to claim 1, wherein when any one of anabaena is selected for culture, the low-cost cyanobacteria culture medium in the step 6) is mixed according to the volume ratio of the livestock and poultry breeding waste separation diluent to the simple cyanobacteria culture medium JYM of 1: 1.5.
3. The method for culturing nitrogen-fixing cyanobacteria in large quantity at low cost according to claim 1, wherein when any one of the monarda is selected for culturing, the low-cost nitrogen-fixing cyanobacteria culture medium in the step 6) is mixed according to the volume ratio of the livestock and poultry breeding waste separation diluent to the simple nitrogen-fixing cyanobacteria culture medium JYM of 1:1.
4. The method for culturing nitrogen-fixing cyanobacteria in large quantity at low cost according to claim 1, wherein when any one of nostoc is selected for culturing, the low-cost nitrogen-fixing cyanobacteria culture medium in the step 6) is mixed according to the volume ratio of the livestock and poultry breeding waste separation diluent to the simple nitrogen-fixing cyanobacteria culture medium JYM of 9: 1.
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CN107852884B (en) * 2017-12-04 2020-08-11 中国科学院水生生物研究所 Method for improving acidified soil and improving soil by using nitrogen-fixing blue algae
CN108753638B (en) * 2018-04-28 2020-04-17 华南农业大学 Nitrogen-fixing blue algae for producing salicylic acid in rice field and application of nitrogen-fixing blue algae in rice field
CN110028167A (en) * 2019-05-23 2019-07-19 安徽吾悦农业科技有限公司 The method for improving aqueous bio nitrogen fixation effect

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